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Expanding the CRISPR Toolbox with ErCas12a in Zebrafish and Human Cells
Author(s) -
Wesley A. Wierson,
Brandon W. Simone,
Zachary WareJoncas,
Carla M. Mann,
Jordan M. Welker,
Bibekananda Kar,
Michael J. Emch,
Iddo Friedberg,
William A.C. Gendron,
Michael A. Barry,
Karl J. Clark,
Drena Dobbs,
Maura McGrail,
Stephen C. Ekker,
Jeffrey J. Essner
Publication year - 2019
Publication title -
the crispr journal
Language(s) - English
Resource type - Journals
eISSN - 2573-1602
pISSN - 2573-1599
DOI - 10.1089/crispr.2019.0026
Subject(s) - crispr , effector , biology , cas9 , nuclease , genome editing , dna , computational biology , genome engineering , rna , zebrafish , gene , guide rna , genome , genetics , microbiology and biotechnology
CRISPR and CRISPR-Cas effector proteins enable the targeting of DNA double-strand breaks to defined loci based on a variable length RNA guide specific to each effector. The guide RNAs are generally similar in size and form, consisting of a ∼20 nucleotide sequence complementary to the DNA target and an RNA secondary structure recognized by the effector. However, the effector proteins vary in protospacer adjacent motif requirements, nuclease activities, and DNA binding kinetics. Recently, ErCas12a, a new member of the Cas12a family, was identified in Eubacterium rectale . Here, we report the first characterization of ErCas12a activity in zebrafish and expand on previously reported activity in human cells. Using a fluorescent reporter system, we show that CRISPR-ErCas12a elicits strand annealing mediated DNA repair more efficiently than CRISPR-Cas9. Further, using our previously reported gene targeting method that utilizes short homology, GeneWeld, we demonstrate the use of CRISPR-ErCas12a to integrate reporter alleles into the genomes of both zebrafish and human cells. Together, this work provides methods for deploying an additional CRISPR-Cas system, thus increasing the flexibility researchers have in applying genome engineering technologies.

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